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运动发酵单胞菌的两种乙醇脱氢酶。通过差异染料配体色谱法进行纯化、分子表征及生理作用研究

The two alcohol dehydrogenases of Zymomonas mobilis. Purification by differential dye ligand chromatography, molecular characterisation and physiological roles.

作者信息

Neale A D, Scopes R K, Kelly J M, Wettenhall R E

出版信息

Eur J Biochem. 1986 Jan 2;154(1):119-24. doi: 10.1111/j.1432-1033.1986.tb09366.x.

Abstract

The two alcohol dehydrogenases found in Zymomonas mobilis have each been purified using dye-ligand chromatography and affinity elution with nucleotides. The isoenzyme with lower electrophoretic mobility (ZADH-1) is a zinc enzyme with properties essentially similar to preparations described elsewhere. The faster isoenzyme (ZADH-2) accounted for some 90% of the ethanol-oxidizing activity in freshly prepared extracts and corresponded to the iron-activated enzyme previously described. This enzyme was inactivated by zinc; activity could only be retained during purification by including either ferrous ions or cobaltous ions in the buffers. ZADH-2 has relatively low acetaldehyde reductase activity; consequently ZADH-1 is responsible for about half of the physiological activity (acetaldehyde reduction) in Zymomonas cells. Kinetic studies showed that ZADH-2 is activated by ethanol in both reaction directions; a hypothesis for the mechanism of activation is presented. Metal ion analyses of ZADH-2 prepared in the presence of iron or cobalt indicated one atom of the relevant metal per subunit, with no significant zinc content. N-terminal sequence analyses showed that the ZADH-1 has some homology with the Bacillus stearothermophilus enzyme, whereas ZADH-2 resembles the yeast enzyme more closely.

摘要

运动发酵单胞菌中发现的两种乙醇脱氢酶均已通过染料配体色谱法和核苷酸亲和洗脱进行了纯化。电泳迁移率较低的同工酶(ZADH-1)是一种锌酶,其性质与其他地方描述的制剂基本相似。较快的同工酶(ZADH-2)在新鲜制备的提取物中约占乙醇氧化活性的90%,与先前描述的铁激活酶相对应。这种酶被锌灭活;只有在缓冲液中加入亚铁离子或钴离子,活性才能在纯化过程中得以保留。ZADH-2的乙醛还原酶活性相对较低;因此,ZADH-1负责运动发酵单胞菌细胞中约一半的生理活性(乙醛还原)。动力学研究表明,ZADH-2在两个反应方向上均被乙醇激活;提出了一种激活机制的假设。对在铁或钴存在下制备的ZADH-2进行的金属离子分析表明,每个亚基含有一个相关金属原子,锌含量不显著。N端序列分析表明,ZADH-1与嗜热脂肪芽孢杆菌的酶有一些同源性,而ZADH-2与酵母酶更相似。

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